Nociceptin receptor coupling to a potassium conductance in rat locus coeruleus neurones <i>in vitro</i>

Connor, Mark; Vaughan, Christopher W.; Chieng, Billy; Christie, MacDonald J.

doi:10.1111/j.1476-5381.1996.tb16080.x

Cited by 208 publications

(127 citation statements)

References 22 publications

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“…8, 17, and 76) and the fact that morphine promotes desensitization but not internalization could be interpreted as evidence for MOP desensitization of inhibition of I Ca occurring via a mechanism unrelated to the internalization pathway. Agonist-stimulated endocytosis and recycling of MOP is thought to be regulated by phosphorylation of residues in the C-terminal region of the receptor by GRKs (12,13,77), whereas acute desensitization of MOP might involve phosphorylation of a residue in the second intracellular loop (63). A differential ability to induce phosphorylation of these residues could provide a structural basis for the apparent separation between the efficacy for desensitization and internalization evident with morphine.…”

Section: Table II Relative Efficacy For Opioid Agonist Inhibition Of mentioning

confidence: 99%

Opioid Agonists Have Different Efficacy Profiles for G Protein Activation, Rapid Desensitization, and Endocytosis of Mu-opioid Receptors

Borgland

Connor

Osborne

et al. 2003

Journal of Biological Chemistry

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144

179

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The differential ability of various -opioid receptor (MOP) agonists to induce rapid receptor desensitization and endocytosis of MOP could arise simply from differences in their efficacy to activate G proteins or, alternatively, be due to differential capacity for activation of other signaling processes. We used AtT20 cells stably expressing a low density of FLAG-tagged MOP to compare the efficacies of a range of agonists to 1) activate G proteins using inhibition of calcium channel currents (I Ca ) as a reporter before and after inactivation of a fraction of receptors by ␤-chlornaltrexamine, 2) produce rapid, homologous desensitization of I Ca inhibition, and 3) internalize receptors. Relative efficacies determined for G protein coupling were [Tyr-D-Ala-Gly-MePhe-Glyol]enkephalin (DAMGO) (1) > methadone (0.98) > morphine (0.58) > pentazocine (0.15). The same rank order of efficacies for rapid desensitization of MOP was observed, but greater concentrations of agonist were required than for G protein activation. By contrast, relative efficacies for promoting endocytosis of MOP were DAMGO (1) > methadone (0.59) > > morphine (0.07) > pentazocine (0.03). These results indicate that the efficacy of opioids to produce activation of G proteins and rapid desensitization is distinct from their capacity to internalize -opioid receptors but that, contrary to some previous reports, morphine can produce rapid, homologous desensitization of MOP.Tolerance to the analgesic and other effects of opioid drugs, such as morphine, undermines their use in long term treatment (1). Although analgesic tolerance is likely to be a complex phenomenon, an understanding of how -opioid (MOP) 1 receptors are regulated by opioid agonists will lead to important insights into this phenomenon. MOPs are similar to many other G protein-coupled receptors (GPCR) in that they undergo desensitization within several minutes of stimulation by agonists (2-4), and continued agonist exposure results in removal of receptors from the cell surface (5-7). MOP phosphorylation is increased as a consequence of agonist exposure, leading to a commonly held assumption that receptor phosphorylation is essential for MOP desensitization and internalization (5, 8 -10). The mechanism that may be responsible for uncoupling MOP from G protein activation and then promoting receptor sequestration is as follows: phosphorylation of the agonist occupied MOP by a G protein receptor kinase (GRK), subsequent binding of ␤-arrestins to the phosphorylated receptor, and removal of MOP from the cell surface via a clathrin-dependent process (11-15). The enhanced analgesic potency of morphine and diminished analgesic tolerance in ␤-arrestin2 knockout mice suggest that the capacity of opioid agonists to cause receptor desensitization and endocytosis is one of the key cellular mechanisms underlying tolerance (16). Phosphorylation of MOP by protein kinase C (PKC) or calmodulin-dependent kinase II can also reduce the capacity of MOP to activate G proteins (8,17), also contributing to opioid tole...

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Section: Table II Relative Efficacy For Opioid Agonist Inhibition Of mentioning

confidence: 99%

Opioid Agonists Have Different Efficacy Profiles for G Protein Activation, Rapid Desensitization, and Endocytosis of Mu-opioid Receptors

Borgland

Connor

Osborne

et al. 2003

Journal of Biological Chemistry

Self Cite

144

179

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“…Interestingly, this fourth member of the opioid receptor family is also coupled to the same second messenger systems [9,10,22,42,57,61,66,70,78,97]. Thus, activation of the ORL-1 receptor leads to inhibition of the enzyme adenylate cyclase [61,78] and calcium channel conductance [10,42,57].…”

Section: Introductionmentioning

confidence: 99%

“…Thus, activation of the ORL-1 receptor leads to inhibition of the enzyme adenylate cyclase [61,78] and calcium channel conductance [10,42,57]. Stimulation of the ORL-1 receptor also activates inwardly rectifying potassium channels [9,97].…”

Section: Introductionmentioning

confidence: 99%

Buprenorphine: A Unique Drug with Complex Pharmacology

Lutfy

Cowan²

2004

280

232

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Buprenorphine, an opioid with mixed agonist-antagonist activity at classical opioid receptors, has been approved recently for the treatment of opioid dependency. Buprenorphine is also used as an analgesic. The buprenorphine dose-response curve is sometimes submaximal, or even bell-shaped, in nociceptive assays, depending upon the nature and intensity of the noxious stimulus. Moreover, buprenorphine, when administered with full agonists, such as morphine, antagonizes the action of these drugs. Partial agonism at the mu opioid receptor and, in some cases, antagonism at the kappa or delta opioid receptor have been considered as possible underlying mechanisms for the ceiling effect and bell-shaped dose-response curve of buprenorphine. While ceiling effects can be explained by partial agonist activity of buprenorphine, the bell-shaped dose-response curve cannot be a consequence of this property of the drug. Recently, buprenorphine has been shown to activate the opioid receptor-like (ORL-1; also known as NOP) receptor. Supraspinal activation of the ORL-1 receptor counteracts the antinociceptive and rewarding actions of morphine, raising the possibility that these actions of buprenorphine can also be altered by its ability to concomitantly activate the ORL-1 receptor. The use of molecular biological techniques has advanced our knowledge regarding the role of opioid receptors in modulation of pain and reward. In particular, generation of opioid receptor knockout mice has proven useful in this regard. Indeed, using knockout mice, we have recently shown that the antinociceptive effect of buprenorphine mediated primarily by the mu opioid receptor is attenuated by the ability of the drug to activate the ORL-1 receptor. Thus, the goal of this review is to provide evidence demonstrating that the ORL-1 receptor plays a functional role not only in the antinociceptive effect of buprenorphine but also in other actions of the drug as well.

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“…Despite these observations, the cellular actions of NC are similar to those of opioids. NC activates the NC-receptor to either inhibit adenylyl cyclase (Meunier et al, 1995;Reinscheid et al, 1995) and/or voltage-gated calcium channels (Connor et al, 1996b;Abdulla & Smith, 1997) or to stimulate an inwardly rectifying potassium conductance (Matthes et al, 1996;Connor et al, 1996a;Vaughan & Christie, 1996). These actions are expected to reduce neuronal excitability and neurotransmitter release.…”

Section: Introductionmentioning

confidence: 99%

Comparison of the effects of [Phe¹Ψ(CH₂‐NH)Gly²]Nociceptin (1–13)NH₂ in rat brain, rat vas deferens and CHO cells expressing recombinant human nociceptin receptors

Okawa

Nicol

Bigoni

et al. 1999

British J Pharmacology

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Nociceptin(NC) is the endogenous ligand for the opioid receptor like‐1 receptor (NC‐receptor). [Phe1ΨC(CH2‐NH)Gly2]Nociceptin(1–13)NH2 ([F/G]NC(1–13)NH2) has been reported to antagonize NC actions in peripheral guinea‐pig and mouse tissues. In this study, we investigated the effects of a range of NC C‐terminal truncated fragments and [F/G]NC(1–13)NH2 on NC receptor binding, glutamate release from rat cerebrocortical slices (rCX), inhibition of cyclic AMP accumulation in CHO cells expressing the NC receptor (CHONCR) and electrically evoked contractions of the rat vas deferens (rVD). In radioligand binding assays, a range of ligands inhibited [125I]‐Tyr14‐NC binding in membranes from rCX and CHONCR cells. As the peptide was truncated there was a general decline in pKi. [F/G]NC(1–13)NH2 was as potent as NC(1–13)NH2. The order of potency for NC fragments to inhibit cyclic AMP accumulation in whole CHONCR cells was NCNH2NC=NC(1–13)NH2>NC(1–12)NH2>>NC(1–11)NH2. [F/G]NC(1–13)NH2 was a full agonist with a pEC50 value of 8.65. NCNH2 and [F/G]NC(1–13)NH2 both inhibited K+ evoked glutamate release from rCX with pEC50 and maximum inhibition of 8.16, 48.5±4.9% and 7.39, 58.9±6.8% respectively. In rVD NC inhibited electrically evoked contractions with a pEC50 of 6.63. Although [F/G]NC(1–13)NH2, displayed a small (instrinsic activity α=0.19) but consistent residual agonist activity, it acted as a competitive antagonist (pA2 6.76) in the rVD. The differences between [F/G]NC(1–13)NH2 action on central and peripheral NC signalling could be explained if [F/G]NC(1–13)NH2 was a partial agonist with high strength of coupling in the CNS and low in the periphery. An alternative explanation could be the existence of central and peripheral receptor isoforms. British Journal of Pharmacology (1999) 127, 123–130; doi:10.1038/sj.bjp.0702539

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Nociceptin receptor coupling to a potassium conductance in rat locus coeruleus neurones in vitro

Cited by 208 publications

References 22 publications

Opioid Agonists Have Different Efficacy Profiles for G Protein Activation, Rapid Desensitization, and Endocytosis of Mu-opioid Receptors

Opioid Agonists Have Different Efficacy Profiles for G Protein Activation, Rapid Desensitization, and Endocytosis of Mu-opioid Receptors

Buprenorphine: A Unique Drug with Complex Pharmacology

Comparison of the effects of [Phe¹Ψ(CH₂‐NH)Gly²]Nociceptin (1–13)NH₂ in rat brain, rat vas deferens and CHO cells expressing recombinant human nociceptin receptors

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Nociceptin receptor coupling to a potassium conductance in rat locus coeruleus neurones in vitro

Cited by 208 publications

References 22 publications

Opioid Agonists Have Different Efficacy Profiles for G Protein Activation, Rapid Desensitization, and Endocytosis of Mu-opioid Receptors

Opioid Agonists Have Different Efficacy Profiles for G Protein Activation, Rapid Desensitization, and Endocytosis of Mu-opioid Receptors

Buprenorphine: A Unique Drug with Complex Pharmacology

Comparison of the effects of [Phe1Ψ(CH2‐NH)Gly2]Nociceptin (1–13)NH2 in rat brain, rat vas deferens and CHO cells expressing recombinant human nociceptin receptors

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Comparison of the effects of [Phe¹Ψ(CH₂‐NH)Gly²]Nociceptin (1–13)NH₂ in rat brain, rat vas deferens and CHO cells expressing recombinant human nociceptin receptors